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α-Glucuronidase and Other Hemicellulase Activities of Fibrobacter succinogenes S85 Grown on Crystalline Cellulose or Ball-Milled Barley Straw

机译:结晶纤维素或球磨大麦秸秆上生长的丁二酸根瘤菌S85的α-葡萄糖醛酸酶和其他半纤维素酶活性

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摘要

Fibrobacter succinogenes produces an α-glucuronidase which cleaves 4-O-methyl-α-d-glucuronic acid from birch wood 4-O-methyl-α-d-glucuronoxylan. Very low levels of α-glucuronidase activity were detected in extracellular enzyme preparations of F. succinogenes on birch wood xylan substrate. The release of 4-O-methyl-α-d-glucuronic acid was enhanced when the birch wood xylan substrate was predigested by either a purified Schizophyllum commune xylanase or a cloned F. succinogenes S85 xylanase. These data suggest that the α-glucuronidase is unable to cleave 4-O-methyl-α-d-glucuronic acid from intact xylan but can act on unique low-molecular-weight glucuronoxylan fragments created by the cloned F. succinogenes xylanase. The cloned xylanase presumably must account for a small proportion of the indigenous xylanase activity of F. succinogenes cultures, since this xylanase source does not support high glucuronidase activity. The α-glucuronidase and associated hemicellulolytic enzymes exhibited higher activities in culture fluid from cells grown on ball-milled barley straw than in that of cellulose-grown cells. The profile of xylanases separated by isoelectric focusing (zymogram) of culture filtrate from cells grown on barley straw was more complex than that of culture filtrates from cells grown on cellulose. These data demonstrate that F. succinogenes produces an α-glucuronidase with an exacting substrate specificity which enables extensive cleavage of glucuronic acid residues from xylan as a consequence of synergistic xylanase action.
机译:琥珀酸纤维杆菌产生α-葡糖醛酸糖苷酶,其从桦木4-O-甲基-α-d-葡糖醛酸木聚糖中切割4-O-甲基-α-d-葡糖醛酸。在桦木木聚糖底物上,琥珀酸镰刀菌的胞外酶制剂中检测到非常低水平的α-葡萄糖醛酸酶活性。当桦木木聚糖底物被纯化的裂殖酵母公社木聚糖酶​​或克隆的丁二酸短杆菌基因S85木聚糖酶预消化时,4-O-甲基-α-d-葡萄糖醛酸的释放得到增强。这些数据表明,α-葡糖醛酸糖苷酶不能从完整的木聚糖上切割4-O-甲基-α-d-葡糖醛酸,但是可以作用于由克隆的琥珀酸木聚糖酶木聚糖酶产生的独特的低分子量葡糖醛酸木聚糖片段。据推测,克隆的木聚糖酶必须占丁二酸琥珀酸菌培养物固有木聚糖酶活性的一小部分,因为这种木聚糖酶来源不支持高葡糖醛酸糖苷酶活性。 α-葡萄糖醛酸苷酶和相关的半纤维素分解酶在球磨的大麦秸秆上生长的细胞的培养液中比在纤维素生长的细胞中显示出更高的活性。通过大麦秆上生长的细胞的培养物滤液的等电聚焦(酶图)分离的木聚糖酶的分布比从纤维素上生长的细胞的培养物滤液的等电聚焦的分布更为复杂。这些数据表明,产琥珀酸短杆菌产生具有严格底物特异性的α-葡糖醛酸糖苷酶,其由于木聚糖酶的协同作用而使得能够从木聚糖中广泛切割葡糖醛酸残基。

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